Agent for gene transfer

ABSTRACT

The invention disclosed and claimed herein is directed toward an agent for the transfer of genetic material comprising a genetic material, PEG-containing liposomes, one or more additional polymer particles and a contrasting agent. The gene transfer agent is particularly suitable for in vivo gene transfer and gene therapy. The invention also is directed toward methods of preparing the agent, and methods of using the agent to affect gene transfer.

[0001] The invention relates to an agent for the gene therapy of tumor diseases and neurodegenerative, cardiovascular and autoimmune diseases. Areas of application for the invention are medicine and the pharmaceutical industry.

[0002] After bronchial carcinoma in men and breast tumors in women, tumors of the large intestine and the colon are the malignant tumors, which occur most frequently in Germany. For these patients, the essential therapeutic measure consists of the radical resection of the tumor-carrying section of the intestine. However, metastasizing (primarily liver metastasizing) is the main cause of the high mortality of colorectal carcinoma. When surgical treatment of the metastases no longer is possible, intensive chemotherapy generally remains the last means of choice.

[0003] In spite of intensive research of new potent chemotherapeutic agents, the treatment of tumors that cannot be resected, especially of liver metastases, continues to be a problem because colorectal carcinoma have a low cell proliferation rate, a tumor heterogeneity and a resistance to drugs. A different reason for the frequent failure of chemotherapy lies therein that the cytostatic agents, presently available, do not attack certain metabolic paths of tumors selectively nor are directed exclusively against tumor cells. Consequently, the use of cytostatic agents is associated with many severe side effects.

[0004] The use of liposomes and polymers offers the possibility of modifying the pharmacological properties of chemotherapeutic agents.

[0005] In spite of decades of intensive efforts to heal patients with inoperable tumors with the help of chemotherapy, progress must be described as slight. With the exception of a few diseases (such as acute lymphatic leukemia) complete healing of the patients by chemotherapeutic measures alone is not possible. In many cases, no significant increase in the life expectancy can be detected. This is due, on the one hand, to the slight tumor specificity of many chemotherapeutic agents and, on the other, to the relatively high toxicity of these substances. Consequently, in spite of massive side effects, an adequate activity level can be observed only rarely in the tumor. In 28 different studies, a total of 663 patients were treated with 22 different substances. Only six patients showed a complete tumor regression and 63 a temporary one which, however, in most cases did not lead to a significant prolongation in the survival time. These studies confirm clearly the need for improving existing therapy concepts and, optionally, for developing new starting points.

[0006] Because of their similarity to cell membranes, liposomes have been used for 23 years as multifunctional carrier and transporting systems for biologically active substances, including prokaryontic and eukaryontic genes (Kim, S., Drugs, 1993, 46: 618-638). They can be characterized as closed microscopic structures, which consist of concentrically disposed lipid double layers, which in turn separate aqueous compartments from one another. Particularly extensive is the work dealing with the liposomal encapsulation of medicinal drugs. In comparison to other carrier systems, the liposomes offer the advantage here that they can be utilized also for the encapsulation of DNA constructs.

[0007] The ability to select the composition, charge, size and stability, depending upon the problem that is to be solved.

[0008] The possibility of complete biological degradation.

[0009] The practical absence of immunological and toxic reactions.

[0010] The frequently changed pharmacokinetics of the liposomally encapsulated substance.

[0011] The changed organ distribution and tropism to certain organs.

[0012] The possibilities for different methods of targeting (antibodies, lectins)

[0013] Liposomes can also be used as gene-transfer systems.

[0014] However, in the majority of animal experimental models, the gene transfer was carried out ex vivo. The knowledge concerning a tumor-specific immune response, induced by the gene-modified tumor cells and obtained by these means, has led to the strategy of a “vaccination” with cytokinin-gene transfected tumor cells. An in vivo gene transfer strategy was employed within the scope of an RAC-approved study at the University of Michigan Medical Center, Ann Arbor. The transfer of an MHC class I (HLA-B7) gene into the tumor cells was to be achieved by the direct injection of liposomes/plasmid DNA complexes into the tumor tissue, in order to stimulate an immune reaction by these means. Other gene transfer systems make use of suicides genes, in order to make tumor cells sensitive to chemotherapeutic substances. Different genes, which can cause a selective killing of the expressed cells, have been tested for this purpose.

[0015] A simple and, according to first clinical data, also effective system was developed by K. Culver (Culver, K. W. et al., Science 1992, 256: 1550) and has already been employed in clinical studies. The strategy is based on the transfer of the herpes simplex thymidine kinase (HSV-tk) gene into tumor cells by means of a retroviral vector. HSV-tk-transfected cells become sensitive to the anti-virus substance ganciclovir. Due to HSV-tk, ganciclovir becomes a nucleotide-like precursor which, after further phosphorylization, is incorporated into the DNA-dividing cells and leads to a stop in the symphysis of DNA and to the death of the cell.

[0016] By means of an adaptation of the Culver suicide strategy to the liver metastasis model and after injection of HSV-tk vector-producing cells, Caruso et al. (Proc. natl. Acad. Sci., 1993, 90: 7024-7028) was able to confirm a regression of established, macroscopically visible liver metastases. However, it is a disadvantage of this application of a tumor therapy with viral vectors that, because of the immunological defense mechanism of the organism, only a single administration of the gene vector construct is possible. For a liposomal vector, repeated systemic processing is possible.

[0017] For the treatment of tumors, the access to which is relatively difficult (such as multiple liver metastases, brain tumors), the selective and safe application and transfection with retroviral or adenoviral vectors still is a problem, quite apart from the treatment risks, which occur with viral infections. As little as possible of healthy tissue should be destroyed and involved, while the transfer efficiency is as high as possible and the subsequent tumor regression is complete.

[0018] Until now, no liposomally packaged therapy gene or suicide gene has been transfected in liver metastases at the CC531 carcinoma.

[0019] It is an object of the invention to supply completely new starting points for a loco-regional treatment of tumors, especially of liver metastases, by a combined use of liposomes/plasmid DNA complexes of different composition, size and loading.

[0020] The object of the invention is accomplished by the distinguishing features described in claims 1, 23 and 25; the dependent claims are preferred variations.

[0021] The core of the invention is a pharmaceutical agent comprising

[0022] one or more genetic materials, not encapsulated or encapsulated in PEG-, immuno-, immuno/PEG-, cationic, optionally polymer-modified liposomes,

[0023] lyophilized or degradable starch particles and/or gelatin and/or polymer particles, such as nanoparticles and

[0024] iodine-, gadolinium-, magnetite-or fluorine-containing contrasting agents.

[0025] Genetic materials preferably are DNA, RNA, ribozyme, antisense oligonucleotides and, especially preferably, therapy genes, such as suicide genes, cytokin genes, chemokin genes (MIP1α, MCP), antiangiogenesis genes, such as vascular endothelial growth factor (VEGF), apoptose genes, such as apoptin, natural born killer (NbK), optionally in combination with marker genes, such as green fluorescence protein (GFP), galactosidase gene (LacZ) under optionally inducible, optionally tissue-specific promoters.

[0026] A further variation of the agent consists therein, that it additionally contains the proteins, which pack DNA more tightly, such as nuclear capsid protein (NCP 7), HMG and/or synthetic substances, such as polyethylene imine, poly-L-lysine or protamine sulfate.

[0027] Preferred suicide genes are herpes simplex virus thymidine kinase gene (HSVtk), deaminase gene, NR/CB1954, pyrine nycleoside phosphorylase and/or the cytokinin genes IL-2, IL-4, IL-6, IL-10, IL-12 and/or IL-15.

[0028] The liposomes consist of

[0029] a) a natural, semi-synthetic or completely synthetic amphiphil

[0030] b) a steroid,

[0031] c) a charged lipid component,

[0032] d) the water-or lipid-soluble genetic material and/or

[0033] e) a carrier liquid and optionally additional inert materials.

[0034] The quantitative ratio of a to b to c preferably is in the molar ratio of 1:0.3:0.1 to 1:1:0.1 or 1:1:0.5 and the molar ratio of c to d is 2:1 to 10:1.

[0035] The natural, semi-synthetic or fully synthetic amphiphil preferably is a lipid, a surfactant, an emulsifier, polyethylene glycol (PEG) or lipid-PEG, the amphiphil being a compound of the general formula I

[0036] in which R₁ and R₂ represent C₁₀ to C₂₀ alkanoyl, alkenoyl, alkyl or alkenyl.

[0037] The steroid used is cholesterol, diethoxycholesterol or sitosterol.

[0038] The charged lipid component is the anion of diacetyl phosphate, of palmitic acid or of stearic acid, the anion of a phospholipid, such as phosphatidyl serine, phosphatid acid or the anion of a sphingolipid, such as sulfatid, or polyethylene glycol (PEG), such as MPEG-DSPE.

[0039] A preferred embodiment of the agent consists therein that the charged lipid component is fluorinated.

[0040] Furthermore, as additional inert materials, polymer particles in the form of a 25% aqueous solution of Poloxamer can be used.

[0041] Preferably, the genetic materials are present in

[0042] SUV (small unilamellar vesicles) PEG liposomes,

[0043] LUV (large unilamellar vesicles) PEG liposomes,

[0044] REV (reverse phase evaporation vesicles) PEG liposomes,

[0045] MLV (multilamellar vesicles) PEG liposomes,

[0046] anti-Ki-67-immune PEG liposomes,

[0047] anti-CEA PEG liposomes or

[0048] PEG DAC-Chol liposomes.

[0049] On the average, the starch particles, preferably lyophilized, are present in a size of 40-90 μm and are in a physiological salt solution in a concentration of 5 to 70 mg/mL. It is especially preferred if the starch particles have a particles size of 60 to 90 μm.

[0050] The inventive agent contains, as iodine-containing contrasting agent, phenyl derivatives with one or more iodine substituents, such as preferably lopromide, loxitalamate, loxaglate, lopamidol, lohexol, lotralon, Metrizamide or Ultravis.

[0051] Fluorinated lipids also come into consideration as contrasting agents.

[0052] A very suitable embodiment is an agent, which contains 30 to 90 mg of lyophilized or degradable starch particles and 5 to 100 mg of genetic material, which is or is not encapsulated.

[0053] A particularly preferred embodiment of the agent is characterized in that it contains

[0054] the LacZ marker gene and the pUT HSVtk suicide gene,

[0055] encapsulated in MLV PEG,

[0056] as starch particles, Spherex or Gelfoam and

[0057] a fluorinated contrasting agent.

[0058] The agents are prepared in that 30 to 90 mg of the lyophilized or degradable starch particles and/or gelatin and/or polymer particles are dissolved in 3 to 6 mL of contrasting agent and afterwards the therapeutically necessary amount of a genetic material is added.

[0059] Preferably, the therapeutic amount of a genetic material and optionally a complexing agent is dissolved in one or several lipids and treated with starch particles and a contrasting agent.

[0060] The inventive agent is used for gene transfer and gene therapy, especially for the therapy of liver metastases, tumors of the lung, bladder, head and neck, urogenitals, lymph nodes, breasts, and in the case of glioblastomata, arthritis and asthma.

[0061] It can equally well be used for local gene therapy.

[0062] In particular, the agent is used

[0063] for the intraarterial therapy of liver metastases, pancreatic tumors, metastases in the pelvis,

[0064] for the treatment of neurodegenerative and autoimmune diseases,

[0065] for Parkinson's and Alzheimer's diseases and for multiple sclerosis,

[0066] in the case of diabetes type I,

[0067] to accompany transplantations,

[0068] for the treatment of restenosis and

[0069] for high blood pressure.

[0070] In summarizing, it is noted once again that the following relationships are of decisive importance for the effectiveness of the inventive liposomes/plasmid DNA complexes.

[0071] 1. The use of the arterial embolization therapy: (direct access to the tumor supply (75-90%), high local tumor concentration and low systemic toxicity)

[0072] 2. The combined use of DNA-carrying liposomes with the embolisate (triple carrier system)

[0073] 3. The use of an effective (strong) promoter.

[0074] It should be emphasized as a special advantage that the organism shows hardly any immunological reaction when this liposome/plasmid DNA complex is used (the unlimited, repeated use is possible); moreover, it was not possible to detect any toxicity.

[0075] The invention will be described in the following by means of examples.

[0076] Method:

[0077] The in vivo Investigation for the Treatment of Liver Metastases in the Animal Model.

[0078] Multi-lamellar polyethylene glycol liposomes (MLV PEG liposomes) are charged with DNA (suicide gene) and, together with the drug carrier embolization system (DCES), are used intraarterially for the treatment of liver metastases in rats.

[0079] Animals:

[0080] For the animal investigations, male Wag/Rij rats where used (bred by: Harlan Winkelmann GmbH, Gartenstrasses 27, D-33178 Borchen). The average weight of the animals is 250-280 g. The animals are kept in accordance with the guidelines of the Animal Protection Law, that is, the specifically pathogen-free (SPF) rats are kept under standardized environmental conditions in the trans-genetic tract of the animal laboratory of the Max-Delbrück center, Berlin-Buch. In the animal cages, the temperature is 22° C. (±1° C.), the relative humidity is 50% (±10%) and the light-dark rhythm is 6 a.m. to 6 p.m.) changed every 12 hours. In a standardized cage (type 3), with a bottom area of 810 cm² and a height of 19 cm, the rats are kept in pairs on a litter of wood shavings (autoclaved at 121° C. for 12 minutes). As standard feed, the animals receive the experimental diet for rats of Firma Sniff, as well as water ad libitum.

[0081] Cell Culture:

[0082] The CC531 cell line is cultured in an RPMI 1640 medium. The medium contains 10% fetal calf serum, 100 U/mL of penicillin G, 100 μg/mL of streptomycin sulfate and 0.25 μg of amphoterizine. The cells are incubated in the incubator at 5% carbon dioxide, 95% relative humidity and a temperature of 37C.

[0083] Preparation of the Liposomes:

[0084] Hydrogenated soybean phosphatidyl choline, cholesterol and polyethylene glycol are dissolved in chloroform in a molar ratio of 1:1:0.1. In the rotary evaporator, the chloroform is evaporated completely from this solution and a lipid film is formed. The lipid film is incubated with distilled water for 12 hours with shaking. During the shaking, MLV PEG liposomes are formed. For preparing the liposomes/DNA complex, the desired concentration of DNA is added to the distilled water phase and shaken with the lipid film as described. At the same time, the DNA is deposited between the lipid double layers that are being formed.

[0085] DNA Used: Reporter gene codes the E. coli lacZ gene (beta-galactosidase), CMV promoter Suicide gene pUT 649 codes the herpes simplex virus thymidine kinase, CMV promoter Suicide gene pBS codes the herpes simplex virus thymidine kinase, CEA-tk CEA promoter

[0086] Preparation and Anesthesia of the Experimental Animals

[0087] The rats are anesthetized for all experimental work. For this purpose, they are placed for about 30 seconds in an ether pot, from which they are removed when immobilization sets in. The injection anesthesias are applied i.m. (into the muscle of the thigh) by means of a 1 mL mixed injection. The further treatment was continued only after the anesthetic and analgesic effect had set in completely after (about 10 minutes). Narcotics Dose 1. Xylazin (Rompun ®, 2%, Bayer AG, 12 mg/kg KGW Leverkusen 2. Ketamine hydrochloride 80 mg/kg KGW (Ketanest ®, 50 mg/mL, PARKE-DAVIS GmbH, Berlin)

[0088] For surgical interventions, the hair on the abdomen was shaved by machine. At the shaved area, the tied up and fixed animals were cleaned and disinfected with 70% ethanol.

[0089] Cell Preparation of the CC531 Cells for the Tumor Inoculation:

[0090] The RPMI medium is aspirated from the cell culture flask and the cell sheet is briefly washed with 3 to 4 mL of trypsin solution. After that, 1 mL (25 cc cell culture flask) or 1.5 mL (75 cc cell culture flask) of trypsin solution is added to the cells and incubated for 10 minutes in the incubator. After that, the flask is taken out and the contents are taken up in 5 mL (25 cc cell culture flask) or 10 mL (75 cc cell culture flask) of RPMI medium. For counting the vital cells, 50 μl of the cell suspension are stained with 50 mL of Trypan blue (alive-dead staining). Because of the increased cell permeability, the dead cells stain blue. Only the vital cells are counted in the Neubauer counting chamber and the count is converted to a figure, equivalent to the total volume.

[0091] The cell suspension is washed twice at 800 to 1000 rpm for 3 to 5 minutes with phosphate-buffered saline (PBS) and then made up to volume with the required amount of PBS (3×10⁵/100 μl of PBS per animal).

[0092] Inoculation of the CC531 Cells:

[0093] The anesthetized rats are opened up in the Linea alba, caudally of the xyphoid. Subsequently, the left liver lobe is advanced. For this purpose, a sterile gauze bandage (5 cm×5 cm) is used, which is soaked in 0.9% sodium chloride solution, in that the liver lobe is carefully taken hold of with the gauze and pulled out about 3 to 4 cm. The advanced portion of the liver is placed on the abdominal wall on moist gauze compresses. The freshly prepared cell suspension (3×10⁵ vital tumor cells in 100 μl of PBS per animal) is injected slowly over a sub-capsular puncture into the left liver lobe (needle: 27G×¼″, No. 20, 0.4×20 mm, TERMUO, Madrid). As the needle is being pulled out, the puncture site is compressed with a cotton swab, in order to prevent the cell suspension flowing away. The puncture opening is then closed off with a drop of tissue adhesive (Histoacryl®, B. Braun Surgical GmbH, Meslungen) and the swab can be removed. The liver lobe is replaced carefully in the abdominal cavity and the abdomen is sutured. Ten to fourteen days after the tumor inoculation, a palpable (approximately 1 cc) tumor has grown in the liver.

[0094] Intraarterial Application of the DNA/Liposome Complexes:

[0095] The abdomen of the anesthetized rats is opened about 5 to 6 cm parallel to the costal arch caudally of the xyphoid. With the help of moistened gauze compresses, the liver portions are displaced cranially and the intestinal portions caudally, so that the lower regions can be observed without hindrance. The further steps take place under microsurgical conditions. Looking through a microscope with 5× to 8× magnification, the A. communis (A. hepatica), A. gastroduodenalis and A. hepatica are exposed.

[0096] A silk thread bridle (5/0, 1 metric, Perma-Hand® silk, braided, ETHICON, Norderstedt) is placed around the A. hepatica propria and the A. gastroduodenalis is ligated distally. Close to the exit of the A. communis, a thread with a loosened knot is placed around the A. gastroduodenalis and subsequently arteriotomized proximally to the ligature. A catheter is introduced carefully through this opening into the vessel and pushed further intravasally. The catheter tube, so placed, is fixed once with the knot previously prepared. Over a hypodermic needle at the other end of the tube, Ringer solution (B. Braun Meslungen AG, Meslungen) is injected (approximately 0.2 mL) under visual control, in order to control the correct discharge of the liquid and the catheter seat in the vessel. After that, the liposomes/DNA complexes are applied (with DCES), alternating with 50 μl of liposomes and 30 seconds of blood flow through the A. communis (loosening the bridled vessel). After the injection is completed, the catheter tube is rinsed once again with Ringer solution (0.2 to 0.3 mL) and pulled out of the vessel. With the previously placed knot, the A. gastroduodenalis can then be tied off proximal to the opening. After that, the gauze compresses are removed and the rats are taken care of further.

[0097] Treatment of the Rats with Ganciclovir:

[0098] Five days after the intraarterial administration of the liposomes/DNA complex, the rats are treated for 14 days with ganciclovir sodium (Cymeven® i.v., Hoffman-La Roche, Grenzach-Wyhlen). For this purpose, 100 mg per kg of body weight of ganciclovir is administered intraperitonally to the animals once daily. For this purpose, the rats were held by the neck with one hand and lifted out of the cage. After an examining aspiration, the rats are injected slowly in the abdomen in the region of the middle line using a 1 mL syringe with a sterile needle (27G×¾″, No. 20, 0.4×20 mm, TERMUO, Madrid).

[0099] Killing the Experimental Animals and Sampling the Blood:

[0100] On the day, on which they are killed, the rats are anesthetized and, after complete analgesia and anesthesia have set in, punctured with a 1 mm syringe (Omnifix®-F, disposable syringe, B. Braun Melsungen AG, Melsungen). For this purpose, the individual animal is placed on its back and, at the level of an imaginary line connecting the two elbows, punctured in the thorax so that the needle (25G×⅝, 0.5×16 mm) is guided to the right of the sternum in the craniodorsal direction. The heart is punctured until the animal dies (approximately 4-6 mL of whole blood).

[0101] The blood obtained is kept for 1 to 2 hours at room temperature or overnight at 4° C. The coagulant formed is then carefully detached from the wall of the tube and centrifuged for 5 minutes at a maximum of 3000 rpm. The supernatant (serum) is then carefully siphoned off and, if necessary, centrifuged once again in order to eliminate admixed erythrocytes. The serum, so obtained, is then deep frozen and kept at −20° C.

[0102] Organ Removal and Preparation:

[0103] The abdomen and thorax of the dead rats are opened and the organs required (liver tumor, liver, kidneys, pancreas, spleen, heart, lung, lymph nodes (from the intestinal mesentery and the axilla)) are removed. All organs are deep frozen at −40° C. with 2-methylbutane (Roth, Karlsruhe) as refrigerant and stored at −70° C.

[0104] Determination of the Size of the Tumor:

[0105] The tumor size is determined using the formula V=a×b²/2, in which a is the largest and b the smallest extent of the tumor. The tumor diameters are measured twice for each animal (day 10 and day 30).

[0106] Serum Analysis:

[0107] The serum samples obtained are analyzed with the Vet Test 8008 (IDEXX GmbH, Wörrstadt, Germany) analytical instrument for veterinary medicine for 16 different blood parameters (photometric measurement), which involved the following substances and enzymes: Substrates Intracellular Enzymes Excretory Enzymes Albumin (g/dl) Creatinine kinase (mg/dl) α-Amylase (IU) Total bilirubin (mg/dl) Aspartate amino Lipase (IU) transferase (IU) Cholesterol (mg/dl) Alanine amino transferase (IU) Creatinine (mg/dl) Lactate dehydrogenase (IU) BUN (urea) (mg/dl) Alkaline phosphatase (IU) Glucose (mg/dl) γ-Glutamyl transferase (IU) Ammonia (mg/dl)

[0108] Preparation of Frozen Section:

[0109] Frozen sections, 8 to 12 μm thick, were prepared from the deep-frozen organs (liver, liver tumor, lung, kidneys, pancreas) using a cryotome (Kryostat of LEICA Instruments GMbH; Nuβloch). The sections were placed on glass microscope slides coated with poly-L-lysine and dried at room temperature. The sections are fixed for 5 minutes in 2% paraformaldehyde solution at 4° C. or for 5 minutes in ice-cold acetone, depending on the further use. The sections are then air dried and stored at −20° C. or stained immediately afterwards.

[0110] Histological Evaluation Hemalum-Eosin Staining (Survey Staining):

[0111] For the histological survey preparations, a double staining with hemalum-eosin is prepared. Basophilic cell structures are stained blue (selective blue staining of the nucleus) by hemalum using the method of Mayer. The plasma is dyed red with the aniline dye eosin Y.

[0112] X-Gal Staining:

[0113] In order to localize the transfected cells and to evaluate the transfer efficiency attained after application of the liposomal pUT651 plasmid, the frozen sections prepared are stained in the following way. The frozen sections, fixed with paraformaldehyde, are washed twice for 5 to 10 minutes in PBS at room temperature and transferred immediately into the freshly prepared incubation solution* and incubated for 4 to 24 hours at 37° C. (development of the blue staining). Subsequently, the sections are rinsed briefly in distilled water and incubated for 30 seconds to 1 minute in eosin. The sections are then dewatered over the increasing alcohol series up to xylene and sealed with Eukitt®.

[0114] Experimental Procedure: Day 0 Tumor 3 × 10⁵ vital CC531 cells in 100 μl of PBS are inoculation injected subcapsular into the liver 10 to 14 A solid 1 cc tumor has grown in the liver days later Day 10 Intraarterial The liposomal DCES with the suicide gene is OP administered over the liver artery Day 15 Ganciclovir Start with the GCV administration (i.p.) 100 mg administered per kg of body weight once daily for 14 days Day 30 Killing with intracardial blood withdrawal

[0115] Reporter Gene Transfer:

[0116] Suicide Gene Transfer:

[0117] Results: Exam- ple Plasmid Liposomes Embolisate Dilution 1 10 μg 50 μl MLV-PEG 100 μl 250 μl Ringer pUT651 Spherex ® solution 2 10 μg 50 μl MLV-PEG 100 μl 250 μl Ringer pUT649 Spherex ® solution 3 20 μg 50 μl MLV-PEG 100 μl 250 μl Ringer pUT649 Spherex ® solution 4 10 μg pBS-tk 50 μl MLV-PEG 100 μl 250 μl Ringer Spherex ® solution Control without without without 250 μl Ringer solution

EXAMPLE 1

[0118] pUT651 (10 μg) is administered to the tumor-carrying rats with the DCES on day 10. Five days later, the expected transfection of the lacZ reporter gene construct is strongest around the tumor and the animals are killed. Subsequently, the organs are removed and worked up as described above. Frozen sections, 12 μm thick, are prepared, fixed with 2% paraformaldehyde solution, washed and incubated at 37° C. overnight in a prepared X-Gal solution. The blue β-galactosidase colored complex can be seen clearly in the region of the edge seam of the tumor. This means that DNA can be transfected selectively with this system in the sensitive growth zone of the tumor. As a rule, no other organs are affected.

EXAMPLE 2

[0119] pUT649 (10 mg) is administered to the tumor-carrying rats with the DCES on day 10. The tumor size is measured during the operation. Five days later, the expected transfection of the suicide gene construct is strongest around the tumor and the GCV administration to the animals is commenced (once daily, 100 mg/kg of body weight). On day 30, the animals are killed. Subsequently, the tumor is measured and blood and organs are removed and worked up as described above. Frozen sections, 12 μm thick, are prepared, fixed with 2% paraformaldehyde solution, washed and stained with the hematoxalyn-eosin stain. The evaluation showed a statistically significant decrease in the liver metastases in comparison to the control group. Complete tumor regression cannot be detected. (See diagram in Appendix)

EXAMPLE 3

[0120] pUT649 (20 mg) is administered to the tumor-carrying rats with the DCES on day 10. The tumor size is measured during the operation. Five days later, the expected transfection of the suicide gene construct is strongest around the tumor and the GCV administration to the animals is commenced (once daily, 100 mg/kg of body weight). On day 30, the animals are killed. Subsequently, the tumor is measured and blood and organs are removed and worked up as described above. Frozen sections, 12 μm thick, are prepared, fixed with 2% paraformaldehyde solution, washed and stained with the hematoxalyn-eosin stain. The evaluation shows a statistically significant decrease in the liver metastases in comparison to the control group. Complete tumor regression cannot be detected. (See diagram in Appendix)

EXAMPLE 4

[0121] pBS-tk (10 mg) is administered to the tumor-carrying rats with the DCES on day 10. The tumor size is measured during the operation. Five days later, the expected transfection of the suicide gene construct is strongest around the tumor and the GCV administration to the animals is commenced (once daily, 100 mg/kg of body weight). On day 30, the animals are killed. Subsequently, the tumor is measured and blood and organs are removed and worked up as described above. Frozen sections, 12 μm thick, are prepared, fixed with 2% paraformaldehyde solution, washed and stained with the hematoxalyn-eosin stain. The evaluation showed that, because of the weaker promoter, a statistically significant decrease in the liver metastases in comparison to the control group, cannot be attained. (See diagram in Appendix)

[0122] Abbreviations:

[0123] CEA Promoter of the carcino-embryonic antigen

[0124] CMV Promoter of the cytomegalo virus

[0125] DCES Drug carrier embolisates system

[0126] HSV-tk Herpes simplex virus thymidine kinase

[0127] i.a. Intraarterial

[0128] i.p. Intraperitoneal

[0129] KGW Body weight

[0130] lacZ gene Reporter gene, codes the β-galactosidase

[0131] MLV PEG Multilamellar vesicles of polyethylene glycol

[0132] OP Operation 

1. A pharmaceutical agent comprising one or more genetic materials, not encapsulated or encapsulated in PEG-, immuno-, immuno/PEG-, cationic, optionally polymer-modified liposomes, lyophilized or degradable starch particles and/or gelatin and/or polymer particles, such as nanoparticles and iodine-, gadolinium-, magnetite-or fluorine-containing contrasting agents.
 2. The agent of claim 1, wherein DNA, RNA, ribozyme and/or antisense oligonucleotides are contained as genetic materials.
 3. The agent of one of the claims 1 or 2, wherein therapy genes, such as suicide genes, cytokin genes, chemokin genes (MIP1α, MCP), antiangiogenesis genes, such as vascular endothelial growth factor (VEGF), apoptose genes, such as apoptin, natural born killer (NbK), optionally in combination with marker genes, such as green fluorescence protein (GFP), galactosidase gene (LacZ) under optionally inducible, optionally tissue-specific promoters, are contained as genetic materials.
 4. The agent of claim 3, wherein the proteins, which packs DNA more tightly, such as nuclear capsid protein (NCP 7), HMG and/or synthetic substances, such as polyethylene imine, poly-L-lysine or protamine sulfate, are contained in addition.
 5. The agent of one of the claims 3 or 4, wherein the agent contains the suicide genes, herpes simplex virus thymidine kinase gene (HSVtk), deaminase gene, NR/CB1954, pyrine nucleoside phosphorylase and/or the cytokinin genes IL-2, IL-4, IL-6, IL-10, IL-12 and/or IL-15.
 6. The agent of one of the claims 1 to 3, wherein the liposomes consist of a) a natural, semi-synthetic or completely synthetic amphiphil, b) a steroid, c) a charged lipid component, d) the water-or lipid-soluble genetic material and/or e) a carrier liquid and optionally additional inert materials.
 7. The agent of claim 6, wherein the quantitative ratio of a to b to c preferably is in the molar ratio of 1:0.3:0.1 to 1:1:0.1 or 1:1:0.5 and the molar ratio of c to d is 2:1 to 10:1.
 8. The agent of claims 6 or 7, wherein the natural, semi-synthetic or fully synthetic amphiphil preferably is a lipid, a surfactant, an emulsifier, polyethylene glycol (PEG) or lipid-PEG
 9. The agent of claim 1, wherein the amphiphil is a compound of the general formula I

in which R₁ and R₂ represent C₁₀ to C₂₀ alkanoyl, alkenoyl, alkyl or alkenyl.
 10. The agent of one of the claims 6 to 9, wherein the steroid is cholesterol, diethoxycholesterol or sitosterol.
 11. The agent of one of the claims 6 to 10, wherein the charged lipid component is the anion of diacetyl phosphate, of palmitic acid or of stearic acid, the anion of a phospholipid, such as phosphatidyl serine, phosphatid acid or the enzyme of a sphingolipid, such as sulfatid, or polyethylene glycol (PEG), such as MPEG-DSPE.
 12. The agent of claim 11, wherein the charged lipid component is fluorinated.
 13. The agent of one of the claims 6 to 12, wherein polymer particles in the form of a 25% aqueous solution of Poloxamer are used as additional inert materials.
 14. The agent of one of the claims 1 to 13, wherein the genetic materials are present in SUV (small unilamellar vesicles) PEG liposomes, LUV (large unilamellar vesicles) PEG liposomes, REV (reverse phase evaporation vesicles) PEG liposomes, MLV (multilamellar vesicles) PEG liposomes, anti-Ki-67-immune PEG liposomes, anti-CEA PEG liposomes or PEG DAC-Chol liposomes.
 15. The agent of one of the claims 1 to 14, wherein the starch particles, lyophilized, are present in a size of 40-90 μm and are in a physiological salt solution in a concentration of 5 to 70 mg/mL.
 16. The agent of claim 15, wherein the starch particles have a particle size of 60 to 90 μm.
 17. The agent of one of the claims 1 to 16, wherein absorbable gelatin powder is contained.
 18. The agent of one of the claims 1 to 17, wherein the agent contains phenyl derivatives with one or more iodine substituents as iodine-containing contrasting agent.
 19. The agent of claim 18, wherein the agent contains lopromide, loxitalamate, loxaglate, lopamidol, lohexol, lotralon, Metrizamide or Ultravis.
 20. The agent of one of the claims 1 to 19, wherein the agent contains fluorinated lipids as contrasting agent.
 21. The agent of one of the claims 1 to 20, wherein the agent contains 30 to 90 mg of lyophilized or degradable starch particles and 5 to 100 mg of genetic material, which is or is not encapsulated.
 22. The agent of one of the claims 1 to 17 and 20 to 21, wherein the agent contains the LacZ marker gene and the pUT HSVtk suicide gene, encapsulated in MLV PEG, as starch particles, Spherex or Gelfoam and a fluorinated contrasting agent.
 23. A method for producing an agent of one of the claims 1 to 22, wherein 30 to 90 mg of lyophilized or degradable starch particles and/or gelatin and/or polymer particles are dissolved in 3 to 6 mL of contrasting agent and, subsequently, the therapeutically necessary amount of genetic material is added.
 24. A method for producing an agent of one of the claims 1 to 22, wherein the therapeutic amount of a genetic material and optionally a complexing agent are dissolved in one or more lipids and mixed with the starch particles and a contrasting agent.
 25. Use of an agent of one of the claims 1 to 22 for gene transfer and gene therapy, especially for the treatment of liver metastases, tumors of the lung, bladder, head and neck, urogenitals, lymph nodes, breasts, in the case of glioblastoma, arthritis and asthma.
 26. The use of claim 25, wherein the agent is used for local gene therapy.
 27. The use of claims 25 or 26, wherein the agent is used for the intraarterial therapy of liver metastases.
 28. The use of an agent of one of the claims 1 to 22 for the treatment of neurodegenerative and autoimmune diseases.
 29. The use of claim 28, wherein the agent is used for Parkinson's disease, Alzheimer's disease and multiple sclerosis.
 30. The use of claim 28, wherein the agent is used for diabetes type
 1. 31. The use of an agent of one of the claims 1 to 22 to accompany transplantations.
 32. The use of an agent of one of the claims 1 to 22 for the treatment of restenosis.
 33. The use of claim 32, wherein the agent is used for high blood pressure. 